Arabidopsis eIF2α kinase GCN2 is essential for growth in stress conditions and is activated by wounding

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Open Access

Research article

Arabidopsis eIF2α kinase GCN2 is essential for growth in stress

conditions and is activated by wounding

Sébastien Lageix

1,3

_{, Elodie Lanet}

2

_{, Marie-Noëlle Pouch-Pélissier}

1

_,

Marie-Claude Espagnol

3

_{, Christophe Robaglia}

2

_{, Jean-Marc Deragon*}

†1

_and

Thierry Pélissier

†1

Address: 1_{Université de Perpignan Via Domitia, CNRS-IRD UMR5096 LGDP, 52 avenue Paul Alduy 66860 Perpignan Cedex, France,}2_Université

Luminy, CNRS-CEA UMR6191 LGBP, 13009 Marseille Cedex 9, France and 3_{Université Blaise Pascal, GReD UMR CNRS 6247, 24 Avenue des}

Landais, 63177 Aubière, France

Email: Sébastien Lageix - Sebastien.LAGEIX@univ-bpclermont.fr; Elodie Lanet - lanet@luminy.univ-mrs.fr; Marie-Noëlle Pouch-Pélissier - marie-noelle.pelissier@univ-perp.fr; Marie-Claude Espagnol - M-Claude.ESPAGNOL@univ-bpclermont.fr;

Christophe Robaglia - robaglia@luminy.univ-mrs.fr; Jean-Marc Deragon* - jean-marc.deragon@univ-perp.fr; Thierry Pélissier - thierry.pelissier@univ-perp.fr

* Corresponding author †Equal contributors

Abstract

Background: Phosphorylation of eIF2α provides a key mechanism for down-regulating protein

synthesis in response to nutrient starvation or stresses in mammalian and yeast cells. However, this process has not been well characterized in plants

Results: We show here that in response to amino acid and purine starvations, UV, cold shock and

wounding, the Arabidopsis GCN2 kinase (AtGCN2) is activated and phosphorylates eIF2α. We show that AtGCN2 is essential for plant growth in stress situations and that its activity results in a strong reduction in global protein synthesis.

Conclusion: Our results suggest that a general amino acid control response is conserved between

yeast and plants but that the plant enzyme evolved to fulfill a more general function as an upstream sensor and regulator of diverse stress-response pathways. The activation of AtGCN2 following wounding or exposure to methyl jasmonate, the ethylene precursor 1-Aminocyclopropane-1-carboxylic acid (ACC) and salicylic acid, further suggests that this enzyme could play a role in plant defense against insect herbivores.

Background

Phosphorylation of the α subunit of eukaryotic transla-tion initiatransla-tion factor 2 (eIF2α) provides a key mechanism for down-regulating protein synthesis in response to nutrient starvation or stresses [1,2]. Vertebrates use four different eIF2α-kinases (PKR, PERK, HRI and GCN2) to respond to various stresses, and typically one kinase has a

predominant role in response to a specific cellular stress condition. For example, in mammals, GCN2 is the pri-mary eIF2α-kinase in response to nutrient limitation [3], PERK modulates gene expression in response to protein misfolding in the endoplasmic reticulum (ER) [4], PKR participates in an antiviral pathway mediated by inter-feron [5], and HRI couples protein synthesis

(predomi-Published: 24 December 2008

BMC Plant Biology 2008, 8:134 doi:10.1186/1471-2229-8-134

Received: 8 September 2008 Accepted: 24 December 2008 This article is available from: http://www.biomedcentral.com/1471-2229/8/134

This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

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BMC Plant Biology 2008, 8:134 http://www.biomedcentral.com/1471-2229/8/134

nantly globin) to the availability of heme in the erythroid cell lineage [6]. However, this specialization of function is not complete and, for example, GCN2 is a secondary eIF2α-kinase in response to ER stress in mouse [7]. Arthropods make a more or less specialized use of eIF2α-kinases. The mosquito Anopheles gambiae has three distinct enzymes (HRI, PERK and GCN2) while Drosophila

mela-nogaster and Caenorhabditis elegans have only two (PERK

and GCN2) [8]. The situation is similar for fungi since

Schizosaccharomyces pombe has three enzymes (two distinct

HRI and a GCN2) while Saccharomyces cerevisiae and

Neu-rospora crassa have a single eIF2α-kinase (GCN2) [8].

In amino acid starved S. cerevisiae cells, GCN2-dependent eIF2α phosphorylation leads to a general down regulation of protein synthesis and to the increased translation of the GCN4 mRNA [2]. Following translation, the GCN4 tran-scriptional activator can induce the transcription of more than 500 genes, including the majority involved in amino acid synthesis. Uncharged tRNAs that accumulate during amino acid starvation activate GCN2 by binding to a his-tidyl-tRNA synthetase-related domain located C-terminal to the kinase domain [2]. S. cerevisiae GCN2 is activated not only by nutrient limitation including amino acid, purine and glucose deprivation, but also by high concen-tration of sodium and by the immunosuppressant rapamycin [2].

In plants, the lower dissociation constant of eIF2 for GDP compared to yeast or mammals have led several years ago to the assumption that plants do not use phosphorylation of eIF2α as a mean to regulate translation [9]. Further-more, the observation that starvation for aromatic or branched amino acids did not initiate a general response have also led to the suggestion that, in contrast to yeast, such general amino acid response may not exist in plants [10]. Therefore the physiological significance of eIF2α phosphorylation in plants is largely unknown. More recently, a GCN2-like enzyme (AtGCN2) has been identi-fied in Arabidopsis thaliana and was shown to restore the growth of a yeast gcn2 mutant in the presence of an inhib-itor of amino acids biosynthesis [11]. AtGCN2 was also shown to be activated in plants by amino acid deprivation conditions [12].

In this work, we show that in response to several stresses, including amino acid and purine starvations, UV, cold shock and wounding, Arabidopsis GCN2 kinase is acti-vated and phosphorylates eIF2α. We show that GCN2 is essential for plant growth in stress situations and that this activity is linked to a strong reduction in global protein synthesis. The activation of GCN2 following wounding or exposure to methyl jasmonate, ACC and salicylic acid, fur-ther suggests that this enzyme could play a role in plant

a key but yet uncharacterized player linking biotic and abiotic stresses.

Results and discussions

Arabidopsis and rice have a single eIF2α kinase

In addition to the presence of a GCN2 enzyme, higher plants have been proposed to contain a double-stranded RNA-dependent protein kinase with biochemical proper-ties of the mammalian PKR [13-15]. Using the protein kinase domain of the yeast and Arabidopsis GCN2 and of the human PKR, PERK and HRI enzymes, we searched the

Arabidopsis genome for the presence of additional eIF2α

kinases. GCN2, PRK, PERK and HRI protein kinase domains were used in a BLASTP analysis against the TAIR 8.0 Arabidopsis proteins http://www.arabidopsis.org and, in each case, fifty proteins with the highest E value were collected. Using this approach, we produced a list of 138 non-redundant kinases (out of the more than 1000

Arabi-dopsis kinases) that most closely resemble eIF2α kinases

(Additional file 1). Using a phylogenetic approach, we compared these 138 kinase domains to yeast, human and mouse eIF2α kinase domains. Two Arabidopsis kinases were found to form a statistically significant cluster with known eIF2α kinases (Additional file 1): one is AtGCN2 (AT3G59410) while the other is annotated as a Wee1-like kinase (AT1G02970) [16]. To evaluate the capacity of the Wee1-like protein to bind to eIF2α, we analyzed in more detail the alignment of this enzyme to the other eIF2α kinases (Additional file 2). We observed that three essen-tial structural characteristics of eIF2α kinases are not present in the Wee1-like kinase: a large insert (more than 30 amino acids) between the conserved kinase domains IV and V [17], a threonine in a putative autophosphoryla-tion site (posiautophosphoryla-tion 446 for the human PKR) [18] and a threonine at the end of domain IX (position 487 for the human PKR) that is critical for the substrate specificity [18]. Therefore, although the Arabidopsis Wee1-like enzyme possess a high degree of homology to eIF2α kinases, as previously noted for the human Wee1 [19], it is unlikely to bind to eIF2α. We conclude that Arabidopsis likely possesses a single eIF2α kinase of the GCN2 type. The same conclusion was obtained using this approach to analyze the rice genome (data not shown) suggesting that higher plants only contain a GCN2-like eIF2α kinase.

Arabidopsis thaliana GCN2 can phosphorylate eIF2α and is essential in amino acid deprivation conditions

To investigate the role of AtGCN2, we first decided to con-firm whether amino acid depletion, a stress known to acti-vate yeast GCN2, is actually inducing eIF2α phosphorylation in Arabidopsis. Similarly to the results recently reported by Zhang et al. [12], we observed that aromatic or branched amino acid deprivation (a situation generated by exposing plants to glyphosate or

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chlorsul-AtGCN2 phosphorylates eIF2α during amino-acid and purine deprivation or after UV irradiation

Figure 1

AtGCN2 phosphorylates eIF2α during amino-acid and purine deprivation or after UV irradiation. A.

Time-course of eIF2α phosphorylation in response to amino acid starvation induced by chlorsulfuron. B. Immunoblot analysis of eIF2α phosphorylation in wild-type (WT) or gcn2 mutant seedlings, untreated (Ø), starved for purine with 8-azaadenine (azA) for 4 h or irradiated with UV. C. Time-course of eIF2α phosphorylation in response to purine starvation induced by azA. D. Time-course of eIF2α phosphorylation in response to UV irradiation. Phosphorylation of eIF2α was measured by using an body that specifically recognizes the phosphorylated form (upper panel). Levels of total protein were assayed by using an anti-body that recognizes tubulin (lower panel).

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tion, an induction that is completely suppressed by adding the appropriate amino acids to the growth medium (data not shown). eIF2α phosphorylation occurs only 4 hours after disrupting the branched amino acid synthesis pathway and peaks after 6 hours of treatment (Figure 1A). eIF2α phosphorylation is completely dependent on the presence of GCN2. Indeed, no phos-phorylation was detected in a GCN2 null mutant line after branched and aromatic amino acid deprivation (Figure 2 and not shown ; see Additional file 3 for a description of the gcn2 mutant line).

In a classical rich medium, gcn2 mutant plants do not have a particular phenotype compared to wild-type plants. However, we observed that gcn2 plants are much more sensitive to chlorsulfuron herbicide treatment than wild-type plants (data not shown). Following 6 days of chlorsulfuron-induced amino acid starvation gcn2 seed-lings appeared smaller and more chlorotic than wild-type seedlings, a result that concurs with that of Zhang et al. [12]. The introduction of an intact copy of AtGCN2 in the gcn2 mutant line allows the plants to grow identically to wild-type seedlings during amino acid deprivation (data not shown), confirming that AtGCN2 is essential for plant growth in this stress situation. As expected, rescue of eIF2α phosphorylation in response to amino acid deprivation was also observed in the complemented gcn2:GCN2 plants (Figure 2). These results confirm that AtGCN2 is the only Arabidopsis kinase involved in eIF2α phosphor-ylation in amino acid starvation conditions.

Characterization of other stresses leading to eIF2α phosphorylation in Arabidopsis

Purine deprivation is known to activate yeast GCN2 [2].

ated by exposing plants to 8-azaadenine (azA) [21]) is also inducing eIF2α phosphorylation in Arabidopsis (Fig-ure 1B). Interestingly, this phosphorylation appears within 2 hours after purine limitation (Figure 1C) and likely results of a reduction in tRNA aminoacylation effi-ciency leading to the accumulation of uncharged tRNAs [2]. eIF2α is also quickly phosphorylated after UV irradia-tion (Figure 1B). This response begins only 20 minutes after irradiation, with a maximum of phosphorylation after 1 hour and a return to basal levels after 6 hours (Fig-ure 1D). Again, both phosphorylation events are com-pletely dependent on the presence of GCN2 as no eIF2α phosphorylation could be detected in the mutant gcn2 line in stress condition (Figure 1B). Although oxidative and osmotic stresses are known to activate yeast GCN2 [2,22], we were not able to activate AtGCN2 using NaCl or H₂O₂(see Figure 3B). Also, heat shock did not lead to eIF2α phosphorylation in Arabidopsis (data not shown) confirming previous results obtained in wheat [23]. In contrast, cold shock, plant wounding, methyl jasmonate, 1-aminocyclopropane-1-carboxylic acid (ACC) and sali-cylic acids were efficient, plant-specific inducer of GCN2-dependent eIF2α phosphorylation (Figure 3 and Addi-tional file 4). Jasmonate acid (JA) and related signaling compounds such as methyl jasmonate are ubiquitous sig-nals for tissue injury and for the subsequent activation of defense response to insect herbivores [24]. ACC is a pre-cursor of ethylene, which also affects the expression of defensive proteins and secondary metabolites in response to insect herbivores [24]. Both ACC and JA accumulate simultaneously in response to insect herbivores and form a conjugate (JA-ACC) that was proposed to coordinately regulate the plant defense response [24]. Finally, salicylic acids is well known to regulate the plant defense response

Molecular complementation of the gcn2 mutant line by the expression of AtGCN2

Figure 2

Molecular complementation of the gcn2 mutant line by the expression of AtGCN2. Immunoblot analysis of eIF2α

phosphorylation in wild type (WT), gcn2 mutant or in three independent gcn2 transgenic lines expressing an intact AtGCN2 (gcn2:GCN2). Seedlings were either untreated (Ø) or starved for branched amino acids with chlorsulfuron (chlor) for 6 hours.

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Stress conditions leading to GCN2-dependent eIF2α phosphorylation in Arabidopsis

Figure 3

Stress conditions leading to GCN2-dependent eIF2α phosphorylation in Arabidopsis. A. Immunoblot analysis of

eIF2α phosphorylation in wild type (WT) or gcn2 mutated seedlings. Seedlings were either left untreated (Ø), starved for purine with azA, exposed to low temperature (cold shock) or wounded on their leaves or roots. B. eIF2α phosphorylation in wild type untreated (Ø) seedlings, or seedlings exposed to NaCl, H₂O₂, low temperature (cold shock), or wounded on their leaves or roots (wound) C. eIF2α phosphorylation in wild type seedlings, untreated (Ø) or exposed to chlorsulfuron, salicylic acid, methyl jasmonate or 1-aminocyclopropane-1-carboxylic acid (ACC). In addition, for methyl jasmonate, eIF2α phosphor-ylation was already detected after 30 minutes of induction (Additional file 4).

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these three key hormones to induce eIF2α phosphoryla-tion suggests that AtGCN2 participates in the plant defense response to insect herbivores.

The AtGCN2 activity is not regulated by the TOR pathway

TOR (target of rapamycin) protein kinase is a central reg-ulator of cell growth in response to nutrient and growth factors [21]. A TOR homolog has been identified in

Arabi-dopsis (AtTOR) and has been implicated in embryo

devel-opment, meristem-driven cell growth, osmotic stress inhibition and the stimulation of mRNA translation [25]. In yeast, phosphorylation of eIF2α by GCN2 is responsi-ble for about 50% of the inhibition of translation initia-tion following the use of the TOR inhibitor rapamycin, suggesting that an important cross-talk exist between TOR and GCN2 pathways [21]. In Arabidopsis, the RNAi inhibi-tion of the TOR pathway also results in a strong inhibiinhibi-tion of translation initiation while TOR overexpressing lines present an increase in translation initiation efficiency [25]. To evaluate the implication of AtGCN2 in this regu-lation, we analyzed the level of eIF2α phosphorylation in AtTOR RNAi-silenced (35-7, 65-1) and overexpressing (G548, G166) lines in normal and amino acid depriva-tion condidepriva-tions (Figure 4). The partly silenced 35-7 and 65-1 lines show a significant decrease in the accumulation of AtTOR mRNA and a severe reduction in shoot and root growth while the two overexpressing G548 and G166 lines have opposite features (increase accumulation of AtTOR mRNA and a strong increase in shoot and root growth) [25]. No increase in eIF2α phosphorylation was detected in unstressed TOR-silenced lines and a similar

silenced and overexpressing lines (Figure 4) suggesting that, in contrast to the yeast situation, no cross-talk exists between the TOR and GCN2 pathways in Arabidopsis.

GCN2 activity induces a strong reduction in global protein synthesis

The impact of eIF2α phosphorylation on the efficiency of mRNA translation was next evaluated. We observed a reduction in the abundance of high-molecular weight polysomes compared to monosomes in amino acids (Fig-ure 5A) or purine (Additional file 5) deprived wild type plants. This variation in the polysomes to monosomes ratio is diagnostic of a reduction in translation elongation rate and translation initiation efficiency caused by these stress conditions. In contrast, we found that amino acids (Figure 5A) or purine (Additional file 5) deprived gcn2 mutant overaccumulates high molecular weight polys-omes compared to monospolys-omes. This suggests that, in these stress conditions, gcn2 mutant can no longer prevent translation initiation in a context where translation elon-gation is slowed down. In support to this conclusion, we observed a marked decrease in the amount of neo-synthe-sized proteins by wild type plant during purine depriva-tion (Figure 5B), a decrease that is much weaker in gcn2 mutant plants (Figure 5B). Globally, these results suggest that the GCN2-dependent increase in eIF2α phosphoryla-tion under amino acids or purine deprivaphosphoryla-tion condiphosphoryla-tions, results in a strong reduction of protein synthesis.

Conclusion

Our data indicate that AtGCN2 is important for plant

The TOR pathway does not interfere with AtGCN2 activity

Figure 4

The TOR pathway does not interfere with AtGCN2 activity. Immunoblot analysis of eIF2α phosphorylation in TOR

RNAi-silenced (35-7 and 65-1) or TOR-overexpressing (G166 and G548) lines (described in [25]). Seedlings of the different backgrounds were either left untreated (Ø) or starved for branched amino acids using chlorsulfuron (Chlor) for 4 h.

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down regulation of mRNA translation. For the moment, it is not known if eIF2α phosphorylation by AtGCN2 can lead to the selective stimulation of specific mRNA transla-tion like this is the case for the yeast GCN4 [2] or mam-malian ATF4 mRNAs [1]. The strong activation of AtGCN2 following wounding and exposure to key hor-mones suggests that this enzyme evolved to play a role in plant defense responses to insect pathogens and may rep-resent a key but yet uncharacterized player linking biotic and abiotic stresses. Therefore, while mammalians use four different eIF2α kinases to respond to a large variety of biotic and abiotic stresses, plants apparently achieve a similar result with a single, GCN2-like enzyme.

Methods

Plant material, growth condition and stress treatments

Wild-type and gcn2 mutated Arabidopsis thaliana plants are from the Landsberg (ler-0) ecotype. The gcn2 insertion

line was obtained from RIKEN Genomic Science Center http://www.riken.jp/engn. Sterile seeds were germinated on solid Murashige and Skoog (MS) medium containing 1% sucrose (w/v) and cultured in a 16-h-light/8-h-dark cycle for 10 days at 23°C. When appropriate, Chlorsul-furon, glyphosate, 8-azaadenine, methyl jasmonate, sali-cylic acid, ACC and branched amino-acid were added to the medium at a final concentration of 0.6 μM, 1.5 mM, 50 μg/ml, 25 μM, 0.6 mM, 50 μM and 5 mM respectively. For the UV stress, seedlings were irradiated with UV light at 50 mJ/m2 by using a UV cross-linker (Bio-Rad Labora-tories, Inc.). Plant wounding was performed by crushing the leaf across the midrib with a haemostat. For the cold shock treatment, seedlings were transferred at 4°C during 2 h followed by 2 h back in the growth chamber at 23°C. Heat shock were performed at 42°C during 2 h followed by 2 h back in the growth chamber at 23°C. For osmotic and oxidative stresses, the seedlings were placed in

solu-AtGCN2 is a regulator of general protein synthesis during amino acids and purine starvation

Figure 5

AtGCN2 is a regulator of general protein synthesis during amino acids and purine starvation. A. Absorbance

pro-file at 254 nm of ribosomes purified by ultracentrifugation on a sucrose density gradient. The ribosomal pellet fraction was pre-pared from wild type (WT) or gcn2 mutant seedlings starved for amino acid using chlorsulfuron for 2 or 4 hours. The positions of the monosomes (80S) and polysomes are indicated. B. 35S-labeled methionine incorporation of wild-type (WT) or gcn2 mutant seedlings starved for purine using azA for 4 to 6 hours. A fraction of the total protein extract was separated on a SDS-polyacrylamide gel, desiccated and exposed to a phosphoimager screen for quantification (upper panel). For each genotype, the relative amount of labeled proteins is indicated under each lane after normalization against the untreated sample set arbitrarily to 1. An equal fraction of the total protein extract was stain with coomassie blue as a loading control (lower panel).

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tions containing 250 mM NaCl or 1 mM H₂O₂during the time indicated.

Immunoblot analysis of eIF2α phosphorylation

Western blots were probed using a phosphospecific anti-eIF2α rabbit monoclonal antibody (Epitomics, Burlin-game, CA; 1/1,000 dilution). After incubation with a horseradish peroxydase-coupled anti-rabbit secondary antibody (Sigma 1/5,000 dilution) immunoblots were developed by using the ECL Plus Western Blotting detec-tion reagents (GE Healthcare Bio-Sciences). Chemilumi-nescence was visualized with a VersaDoc Imaging System (Bio-Rad Laboratories, Inc.). Equal loading of protein were confirmed by reprobing the membranes with a mouse monoclonal anti-alpha-tubulin (Sigma 1/5,000 dilution).

Polysome preparation and detection of neo-synthesized proteins in normal and stress situation

For polysome preparation, seeds were sown in liquid medium, incubated 48 h at 4°C, and grown under con-stant light during 10 days at 23°C. Chlorsulfuron was added, and after 2 or 4 hours, the ribosomal pellet frac-tion was prepared from wild-type (WT) or gcn2 mutant seedlings as described in [25]. Polysome profiles were dis-played on sucrose gradients and profiles recorded at 260 nm. For the detection of neo-synthesized proteins, the 10 days-old seedlings were treated for 2 to 4 hours with 8-azaadenine and then transferred for 2 hours into 1 ml of

MS medium containing 50 μCi of 35_S-labelled

methio-nine and 8-azaademethio-nine. Untreated controls were incu-bated for 2 hours into the same labelling medium, but in the absence of 8-azaadenine. After two washes with MS medium, total proteins were extracted as described below and 35 μg of protein were separated on SDS-PAGE. Gels were stained with Coomassie blue or dried and autoradi-ographied using a PhosphoImager (Bio-Rad Laboratories, Inc.).

Preparation of total protein extracts

Following exposure to stress, total protein extracts were prepared as following. For each treatment, three seedlings were ground in Laemmli buffer containing both Com-plete protease and PhosSTOP phosphatase inhibitor (Roche Diagnostics, Indianapolis, IN) and incubated at 95°C for 5 min. After centrifugation, samples were frac-tioned by sodium dodecyl sulphate-polyacrylamide gel electrophoresis (SDS-PAGE) and transferred to nitrocellu-lose.

Authors' contributions

SL carried out the molecular genetic studies on GCN2, participated in the polysome profile analysis and drafted the manuscript. EL did the polysome profile analysis and,

vided technical help on the molecular genetic work. JMD and TP conceived the study, participated in its coordina-tion and final writing of the manuscript. All authors read and approved the final manuscript.

Additional material

Acknowledgements

This work was supported by the CNRS and the Université of Perpignan.

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Additional file 1

Evolutionary tree of the kinase domains of 138 Arabidopsis enzymes most closely related to GCN2, PKR, PERK and HRI eIF2α kinases.

Click here for file

[http://www.biomedcentral.com/content/supplementary/1471-2229-8-134-S1.pdf]

Additional file 2

Multiple sequence alignment of the kinase domains of the eIF2α kinase group on the evolutionary tree of Additional file 1, performed using MUSCLE (v3.7).

Click here for file

Additional file 3

Description of the gcn2 mutant line.

Click here for file

Additional file 4

Phosphorylation of eIF2α in response to hormones.

Click here for file

Additional file 5

Absorbance profile at 254 nm of ribosomes purified by ultracentrifu-gation on a sucrose density gradient.

Click here for file

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